Deciphering DED assembly mechanisms in FADD-procaspase-8-cFLIP complexes regulating apoptosis

Fas-associated protein with death domain (FADD), procaspase-8, and cellular FLICE-inhibitory proteins (cFLIP) assemble through death-effector domains (DEDs), directing death receptor signaling towards cell survival or apoptosis. Understanding their three-dimensional regulatory mechanism has been limited by the absence of atomic coordinates for their ternary DED complex. By employing X-ray crystallography and cryogenic electron microscopy (cryo-EM), we present the atomic coordinates of human FADD-procaspase-8-cFLIP complexes, revealing structural insights into these critical interactions. These structures illustrate how FADD and cFLIP orchestrate the assembly of caspase-8-containing complexes and offer mechanistic explanations for their role in promoting or inhibiting apoptotic and necroptotic signaling. A helical procaspase-8-cFLIP hetero-double layer in the complex appears to promote limited caspase-8 activation for cell survival. Our structure-guided mutagenesis supports the role of the triple-FADD complex in caspase-8 activation and in regulating receptor-interacting protein kinase 1 (RIPK1). These results propose a unified mechanism for DED assembly and procaspase-8 activation in the regulation of apoptotic and necroptotic signaling across various cellular pathways involved in development, innate immunity, and disease.


mutations
In order to explore the interactions between FADD, Casp-8, and cFLIP that regulate signaling, we generated various combinations to reconstitute the DED core complexes for our structural studies.However, when Casp-8 tDED was overexpressed, it predominantly formed filaments, regardless of the presence of cFLIP or full-length FADD (FADD FuL ), and precipitated in E. coli.This precipitation hindered the reconstitution of multiprotein complexes (Fig. 1a).
Mutations in Casp-8 tDED were employed to increase the population of monomers 38,45,47,50 .For instance, a double mutation, F122A/L123A, targeting the conserved hydrophobic phenylalanine/leucine motif (the FL motif, Supplementary Fig. 1a) on the type Ib surface of Casp-8 DED2, prevented the formation of the death effector filament (DEF) or selffilamentation when overexpressed in HeLa cells 47 .Therefore, we applied a similar strategy to enrich the population of soluble tDED complexes.Notably, the overexpression of the Casp-8 tDED F122A mutant (Casp-8 tDED_F122A ) still led to the formation of apoptotic DEFs 51 and efficient recruitment to the DR5 DISC but impaired TRAIL-induced apoptosis 45 .We observed that co-expression of Casp-8 tDED_F122A and cFLIP tDED H7G mutant (CF H7G ), both of which lack the protease domain, led to a mixture of Casp-8 tDED_F122A DEF filaments and oligomeric CF H7G -Casp-8 tDED_F122A tDED complexes (Fig. 1b).This suggests that cFLIP is capable of inhibiting Casp-8 filamentation but is outcompeted by Casp-8 self-filamentation during overexpression studies.
To further reduce Casp-8 self-filamentation during the reconstitution of DED core complexes, we introduced F122G/L123G double mutations, often referred to as FGLG.Importantly, the Casp-8 tDED_F122GL123G mutant (C8 FGLG ) is predominantly monomeric in gel filtration 38 and exhibits no self-filamentation (Fig. 1c).However, it is capable of forming short filaments in the presence of FADD FuL (Fig. 1c).This observation implies that FADD can still interact with C8 FGLG to induce C8 FGLG filamentation.
Collectively, the results suggest that Casp-8 with mutations in the FL motif or F122 only affect Casp-8 tDED -Casp-8 tDED assembly in Casp-8 tDED filament extension but not FADD DED -Casp-8 tDED and Casp-8 tDED -cFLIP tDED assemblies in the FADD-Casp-8-cFLIP complex.Therefore, these mutations can facilitate the reconstitution of multiprotein DED complexes to unveil these unknown assemblies.As demonstrated by the atomic coordinates we present below, the interaction between FADD and Casp-8 utilizes the type Ib surface of Casp-8 DED2 rather than its FL motif.In addition, the interaction between cFLIP and Casp-8 does not involve the FL-motif containing, type Ib surface of Casp-8.
In the crystal structure, FADD is sub-stoichiometric to Casp-8, consistent with previous observations in CD95 and TRAILR DISCs 46,47 .Our recombinant ternary complex is in agreement with the TRAILR DISC from BJAB cells, which contains a single FADD subunit and a 1:9 ratio of FADD to tDED-containing proteins 47 .If a TRAILR DISC comprises three pairs of TRAILR and TRAIL, a single FADD, and nine fulllength Casp-8 molecules, it would have a molecular weight of ~790 kDa.This aligns with the characterization of a high molecular weight (HMW) DISC, which is >700 kDa, in tumor cells 47 .Therefore, our single-FADD ternary DED complex closely resembles the DED subcomplex within the TRAILR DISC.
Upon our initial examination without crosslinking, we obtained a cryo-EM structure of the FA FuL -C8 FuL_FGLG_CADA -CF complex at 7.5 Å resolution, referred to as Complex A (Supplementary Fig. 5, 6 and Supplementary Table 2).Unexpectedly, this structure revealed a 3:3:4 ratio of FADD-Casp-8-cFLIP DED core complexes, forming what we refer to as a triple-FADD ternary DED complex.However, both Casp-8 protease domain and FADD DD were not visible, suggesting that these two domains didn't form a stable complex.
To validate this observation, we produced a GraFix-stabilized version of the FA FuL -C8 FuL_FGLG_CADA -CF complex and solved the cryo-EM structure at 3.7 Å resolution, named Complex B (Supplementary Figs.5-9 and Supplementary Table 3).Complex B confirmed the 3:3:4 model observed in Complex A (Fig. 2d, f, Supplementary Fig. 2e, and Supplementary Movie 2), with invisible Casp-8 protease domain and FADD DD.
Both Complex A and Complex B exhibit a balanced ~1:1:1 ratio of FADD, Casp-8, and cFLIP within the complex.This ratio aligns with previous observations made in CD95 DISC from cFLIP S -overexpressing BJAB and HaCaT cells 48 and SKW6.4 cells 46 and also in DR5 DISC from A549 and H460 cells 45 .These findings support the notion that our triple-FADD ternary complex closely resembles the DED subcomplexes found in these DISCs.
In both the single-FADD and triple-FADD complexes, Casp-8 tDED consistently utilizes a composite-self-assembling site (CSS) composed of a type II and two type III surfaces (Fig. 2c, f, g), referred to as the type III-II-III CSS (Supplementary Fig. 1b), to form a transient left-handed pentamer (Supplementary Movie 3) and trimer, respectively (Fig. 3c).This emphasizes the importance of the type III-II-III CSS in Casp-8 tDED self-assembly and filament formation, as supported by our results showing that C8 tDED_FGLG can still form short filaments in the presence of FADD (Fig. 1c).
In addition, two FADD DED molecules FAq and FAr (Fig. 4d) assemble like the Casp-8 tDED molecule C8d in the single-FADD complex (Fig. 4f).Together they provide a type II and two type III surfaces, mimicking the type III-II-III CSS, for interaction with Casp-8 tDED molecule C8c (Fig. 4c, d vs. 4e, f).Therefore, to form a triple-FADD complex, the FADD trimer could sequentially recruit three Casp-8 tDED molecules C8c, C8b, and then C8a, via the type III-II-III CSS, as portrayed in Stage 3 of Supplementary Fig. 12a.Alternatively, the FADD trimer could bind simultaneously C8a and C8c of a transient, type III-II-III CSS-mediated Casp-8 tDED trimer, which contains C8a, C8b, and C8c, and stabilize the trimer (Stage 3 of Supplementary Fig. 12a).The FADD DED -FADD DED and FADD DED -Casp-8 tDED interactions unveiled by the atomic coordinates of the triple-FADD complex (Fig. 4a) allow us to propose how FADD DED and Casp-8 tDED assemble a triple-FADD intermediate complex in DRmediated signaling (Supplementary Fig. 12a).
In summary, both triple-FADD and single-FADD structures argue that Casp-8 tDED utilizes the type III-II-III CSS to self-assemble functional oligomers (Supplementary Fig. 12a, b).This may play a significant role, especially considering the abundance of Casp-8 in various cell types 9,52,53 with levels higher than FADD and cFLIP 11,46,54 .It is plausible that high levels of Casp-8 could promote the formation of transient Casp-8 oligomers, contributing to the creation of a FADD-Casp-8 intermediate complex.
It's important to note that endogenous Casp-8 typically does not form filaments automatically in cells; instead, it requires FADD upon DR stimulation.It was believed that a conformational change in FADD was triggered to expose its DED to seed the formation of Casp-8 DED complex 39,52,55 .Our structures argue that the role of exposed FADD DED in seeding may involve stabilizing transient Casp-8 oligomers assembled via the type III-II-III CSS of tDED to complete a FADD-Casp-8 intermediate complex.This intermediate complex can subsequently recruit cFLIP to form an anti-apoptotic ternary complex (Supplementary Movie 5) or Casp-8 to create apoptotic filaments in DR-mediated signaling (Supplementary Fig. 12).This insight explains why C8 FGLG requires FADD to form an intermediate complex for initiating C8 FGLG filamentation (Fig. 1c).
In both intermediate complexes, the first cFLIP tDED that binds the FADD-Casp-8 intermediate complexes should be cFLIP tDED molecule CFk because its interface area, which is >1,650 Å 2 corresponding to a BSA of >3,300 Å 2 with ~38 hydrogen bonds/salt bridges, is much larger than those of cFLIP tDED molecules CFi and CFj, which are ~730 Å 2 (Fig. 2c, f).Therefore, our structures demonstrate that the FADD-Casp-8 intermediate complexes assemble a composite-binding site (CBS) to recruit CFk (Fig. 5a).
Once an upstream cFLIP tDED molecule, for example, CFk, binds the CBS, it, in turn, provides surfaces to assemble the next CBS for recruiting the next cFLIP tDED molecule CFj (Fig. 5b, Supplementary Movie 6).The CBS for recruiting the second cFLIP tDED molecule CFj consists of a type III-II-III CSS from cFLIP tDED molecule CFk and a type Ia and a type IIa surfaces respectively from two Casp-8 tDED molecules C8b and C8c, with an interface area of ~1,400 Å 2 in total (Fig. 5b).The third cFLIP molecule CFi is recruited in a similar way along the type III connectivity (Fig. 5b), via a CBS with an interface area of ~1200 Å 2 .Therefore, the recruitment of cFLIP molecules, either cFLIP L or cFLIP S , would depend on a hierarchical process.In our structures, cFLIP tDED also forms a type III-II-III CSS-mediated trimer.
The CBS for recruiting the fourth cFLIP tDED molecule CFh, with an interface area of ~1300 Å 2 , looks different from aforementioned CBS and has different Casp-8 tDED -cFLIP tDED and cFLIP tDED -cFLIP tDED interactions.Two upstream cFLIP tDED molecules CFk and CFi provide a type Ia and a type IIIa surfaces, respectively, while Casp-8 tDED molecule C8a provides two type IIa and a type IIIa surfaces (Fig. 5b).Notably, despite variations in CBS assembly, all cFLIP tDED -recruiting CBSs are composed of five surfaces, including a type Ia, two type IIa, and two type IIIa surfaces.
Furthermore, because cFLIP S lacks a protease domain, the assembly of a Casp-8 tDED -cFLIP tDED hetero-double layer unequivocally allows only the FADD-Casp-8-cFLIP L complex, but not FADD-Casp-8-cFLIP S , to foster heterodimerization between the protease domains of cFLIP and Casp-8, resulting in local Casp-8 activation for processes like cleaving RIPK1 to inhibit necroptosis 33 .Consequently, our structures also clarify structurally why the recruitment of cFLIP L , but not cFLIP S , to the FADD-Casp-8 intermediate complex (Fig. 2) leads to partial/local Casp-8 activation.Notably, in contrast to Casp-8 in DEF that could fully activate Casp-8 to generate apoptotic Casp-8 heterotetramers 6,31,32 , Casp-8 in the FADD-Casp-8-cFLIP S complex mentioned earlier is inactive.Hence, a single layer of Casp-8, consisting of either a trimer or pentamer, in our FADD-Casp-8 intermediate complexes appears unable to trigger Casp-8 autoactivation.This is likely due to the tDED complex's helical twist of approximately 71 degrees along the type III connectivity, which may hinder the protease domain of Casp-8, shown as prominent red spheres in Fig. 5c, from homodimerization.Therefore, our structures further argue that both cFLIP L and cFLIP S binding to the FADD-Casp-8 intermediate complex would prevent the addition of a second Casp-8 layer and, consequently, the full activation of Casp-8.
In addition, we can postulate that, during DR activation, a shortage of cFLIP would allow the formation of a Casp-8 double layer, setting the stage for the dimerization of Casp-8's protease domains.As mentioned earlier, the type III-II-III CSS-mediated Casp-8 tDED trimer represents the minimum repeating unit (Supplementary Fig. 11a) in the assembly of Casp-8 tDED filaments.A cFLIP shortage-mediated generation of Casp-8 double layer, comprised of two non-apoptotic Casp-8 trimers stacked along the type I connectivity, emerges as a pivotal step in achieving full Casp-8 activation in FADD-mediated or Casp-8 filamentation-mediated apoptotic pathways.

Two unidirectional FADD-mediated Casp-8 filamentation models
Significantly, our EM results reveal that FADD and cFLIP attach to the Casp-8 tDED filaments only at one end (Fig. 1a).However, in our structures, they occupy opposite ends (Fig. 2d).These observations suggest that FADD-induced Casp-8 filamentation is unidirectional, leaving the other end open for cFLIP to physically obstruct it, as discussed earlier.
In fact, the triple-FADD structure demonstrates that FADD can physically impede Casp-8 filamentation at the upper end (Fig. 2e, f).In the single-FADD structure, the halt of Casp-8 filamentation at the upper end results from the inability of the CSS of Casp-8 tDED molecule C8e to bind and stabilize another Casp-8 tDED when there's no FADD in the adjoining space (Fig. 2b, c).Consequently, our structures contribute to our understanding of the mechanism behind FADD-mediated unidirectional Casp-8 filamentation.
In addition, a type IIa and a IIIa surfaces are offered by FADD DED molecule FAl to bind cFLIP tDED molecule CFk, similar to how FADD DED molecule FAq binds Casp-8 tDED molecule C8c in the 3:3:4 FADD-Casp-8-cFLIP complex structure (Supplementary Fig. 10a).The former FADD DED molecule contributes an interface area of around 630 Å 2 , while the latter contributes 500 Å 2 .Therefore, at least four surfaces of the CBS are capable of binding Casp-8 tDED .These four surfaces contribute 1,200 Å 2 of interface area, sufficient for binding a Casp-8 tDED , although no structure shows that the remaining type IIa surface of FADD DED molecule FAr or Casp-8 tDED molecule C8d DED1, depicted as black dotted circles in Supplementary Fig. 10b and 10d, respectively, can bind Casp-8 DED2.
Thus, we propose that during DR activation, in the event of cFLIP shortage, the available Casp-8 in cells would be like Casp-8 tDED molecule C8 1 that targets the CFk-binding CBS on the remaining FADD-Casp-8 intermediate complexes (Supplementary Fig. 10b or 10d), which is like cFLIP tDED would normally do (Supplementary Fig. 10a or  10c).The recruitment of Casp-8 tDED molecule C8 1 would create a CBS identical to the corresponding one in Casp-8 filaments.Consequently, the newly created CBS would recruit the second and third Casp-8, which are Casp-8 tDED molecules C8 2 and C8 3 in Supplementary Fig. 10b, respectively, to complete the second type III-II-III CSS-mediated Casp-8 trimer and hence a Casp-8 double layer.
Importantly, the resultant Casp-8 double layer would also contain a newly created CBS that would initiate the recruitment of more Casp-8, such as Casp-8 tDED molecule C8 4 and beyond, to form the third Casp-8 layer (Supplementary Movie 7).This process generates numerous Casp-8 helical double layers in filament extension for apoptotic Casp-8 activation.By substituting cFLIP tDED in our structures with Casp-8 tDED , we could establish both single-FADD and triple-FADD models (Supplementary Fig. 10b, d) for FADD-mediated unidirectional Casp-8 filamentation.

Triple-FADD model regulates apoptotic signaling in cells
As it's uncertain whether TNFR, CD95, and TRAILR employ similar signaling mechanisms and complexes to activate Casp-8, we aimed to investigate the involvement of our models in hierarchical FADDmediated Casp-8 activation.To do this, we created FADD-knockout (FADD-KO) iMEF cells using the CRISPR-Cas9 system (Supplementary Fig. 15a) and reconstituted FADD with different mutations on the five FADD-tDED interfaces identified in the single-FADD structure.These mutations included type Ia (Q40A), type IIa (E51R), type IIIa (R34A, K33E, E37A), type Ib (E22R, F25R, F25Y), and type IIb (D74A) mutations, indicated by the red, cyan, black, green, and orange boxes in Fig. 6a.We aimed to determine whether these mutations would impair apoptotic signaling.
However, only few FADD-deficient clones survived, and some of them expressed minimal RIPK3 or MLKL, e.g., the clones sg4.4,sg4.5, and sg4.10 in Supplementary Fig. 15a.This could be partially explained by previous observations that the embryonic lethality of FADDdeficient mice could be rescued by ablating RIPK3 to block necroptotic signaling 59 .Hence, the surviving FADD-KO iMEF clones may have a defect somewhere in the FADD-independent necroptotic signaling pathway.It's worth noting that surviving FADD-deficient MEF cells are known to be resistant to TNF-induced necroptosis 60,61 .We selected FADD-KO clone sg4.B9 for further study since it expressed both RIPK3 and MLKL (Supplementary Fig. 15a, lane 2), making it suitable for testing FADD-dependent apoptotic signaling and FADD-dependent RIPK3 activation.
Next, we reconstituted WT FADD and FADD mutants in the FADDdeficient iMEF cells to assess their impact on TNF/CHX-induced apoptosis.Unlike WT FADD, FADD F25R, K33E, E37K, E51R, and R34A mutants hardly restored TNF/CHX-induced Casp-8 activation, as indicated by less production of cleaved Casp-3 (c-Casp-3) (Fig. 6b).Among those mutants, FADD F25R, K33E, and E51R mutants hardly restored TNF/CHX-induced apoptosis (Supplementary Fig. 15c) and Casp-3 activation (Supplementary Fig. 15d).Casp-3 activation was confirmed by zVAD inhibition (Supplementary Fig. 15f).These results suggest that the type IIa (E51), type IIIa (K33), and type Ib (F25) surfaces of FADD are essential for Casp-8 activation and, consequently, apoptosis.Furthermore, because FADD D74 is located on type IIb surface (Fig. 6a, orange box) and is associated only with the single-FADD model, assessing the impact of the FADD D74A mutant on signaling would determine the necessity of FADD D74 and the single-FADD model.The results indicate that the FADD D74A mutant behaves like the WT protein (Fig. 6b, lane 20 vs. 16, Supplementary Fig. 15a, b), suggesting that FADD D74 and the single-FADD model are dispensable for TNF/CHX-induced TNFR1-mediated apoptotic pathways.Consequently, it is inferred that only the triple-FADD model is implicated in these pathways.
We also determined that FADD residues F25, K33, and E51 play crucial roles in TRAIL-induced Casp-8 activation in HAP1 cells (Fig. 6d).However, it remains inconclusive which model or whether FADD D74 was utilized, as the FADD D74A mutant in HAP1 cells was not stable after death induction for an unknown reason (Fig. 6d, lane 20).It is noteworthy that, although a somewhat similar trend is observed in TCand TCZ-treated iMEF cells (Fig. 6b, c, lane 20), FADD D74A mutation did not impact Casp-3 activation, apoptosis, and necroptosis (Supplementary Fig. 15c-e).
The structural breakthrough was achieved by Casp-8 tDED FGLG mutations and overexpressing cFLIP tDED , effectively limiting Casp-8 tDED self-filamentation.Consequently, the ternary DED complexes with a minimum DED assembly was purified homogeneously, leading to improved resolution and atomic model building 40,41 .The resultant minimum DED complex likely mirrors its WT Casp-8 tDED counterpart at certain stage, supported by previous observations where the complex of Casp-8 FGLG mutant is like WT Casp-8 that could cleave RIPK1, possibly in complex with cFLIP L 70 .Notably, Casp-8 tDED FGLG mutations shield other intrinsic DED-DED interactions in the ternary complexes, allowing the identification of CFk as the sole cFLIP tDED molecule that interacts simultaneously with FADD DED and Casp-8 tDED (Fig. 5a, b).Replacing cFLIP tDED molecule CFk (Supplementary Fig. 10a) with a Casp-8 tDED (Supplementary Fig. 10b) would eliminate the sole FADD DED -cFLIP tDED interaction in the complex, potentially initiating apoptosis.
In our atomic coordinates, DED2 of Casp-8 tDED molecule C8a binds to FADD DED molecule FAl, followed by its DED1 binding to DED2 of cFLIP tDED molecule CFi along type I interactions (Fig. 2c, f).Therefore, earlier models, which propose Casp-8 DED1 binds to FADD DED , followed by DED2 binding to the DED1 of the next Casp-8 tDED molecule 39 , may feature reversed orientations of DED2 to DED1 (Supplementary Fig. 11g and Supplementary Movie 8).Alternatively, our structures offer a different model in which cFLIP tDED targets the CBS of the FADD-Casp-8 intermediate complex, with four cFLIP tDED molecules effectively obstructing the bottom-end extension of a Casp-8 tDED trimer (Fig. 5a, b and Supplementary Fig. 13).Notably, since our structures and Casp-8 tDED filament structure (PDB: 5L08) 38 comprise only type III-II-III CSSmediated trimer (Supplementary Fig. 10a, c and 11a), it suggests that Casp-8 tDED may dimerize along type III connectivity to form nonapoptotic type III-II-III CSS dimers (Supplementary Fig. 11b), called offset dimer previously 39 , and trimers in the FADD-Casp-8 intermediate complex.Random dimerization along type II and III connectivity could yield three additional Casp-8 tDED trimers (Supplementary Fig. 11c-e).However, these three trimers would generate apoptotic type II-III-II CSS dimers, also called aligned dimers previosuly 39 , under nonapoptotic condition.Therefore, it is likely that an apoptotic type II-III-II CSS Casp-8 tDED dimer, such as the Casp-8 tDED C8h-C8a dimer (Supplementary Fig. 11a, b, f) and the Casp-8 tDED dimer between N th and (N + 2) th asymmetric units (Fig. 7c), has to appear after the fourth Casp-8 tDED molecule targets the FADD-Casp-8 intermediate complex (Fig. 7b) for a tighter control of apoptosis (Supplementary Movie 7).Future investigations, or a high-resolution map, are necessary to determine whether this model requires further modification.
The observed discrepancy in mutagenesis results indicates that the role of FADD residue F25 differs from that of FADD residue K33, E37, E51, or R34 (Fig. 6b and Supplementary Fig. 15c, d).A single mutation at F25 alters ~20% of the type IIa surface of FADD, a significantly greater change than the ~7% alteration of the CBS surface caused by a single mutation at K33, E37, E51, or R34.The F25R mutation likely disrupts the formation of the triple FADD-Casp-8 intermediate complex.Consequently, both Casp-7 and Casp-3 remain inactive, abolishing subsequent PARP cleavage (Fig. 6b).Conversely, mutations at K33, E37, E51, or R34 lead to partial Casp-3 activation (Fig. 6b), indicating that the FADD-Casp-8 intermediate complex assembles normally, but the ~7% change in the CBS surface results in partial Casp-8 activation.However, PARP cleavage could be attributed to the partial colocalization of Casp-7 and TNF-R1 receptosome 71 , rendering Casp-7 activation and subsequent PARP cleavage insensitive to the ~7% change in the CBS.Additionally, Casp-7 exhibits better efficiency than Casp-3 in cleaving PARP 72,73 .Therefore, adding FADD to HeLa cell lysates could bypass TNF-R1 receptosome, making PARP cleavage sensitive to Casp-3 activation and CBS alterations (Supplementary Fig. 15i).These findings strongly link the formation of both the triple-FADD intermediate complex and CBS to critical processes such as caspase activation, apoptosis, and necroptosis.
It's important to acknowledge that our structures do have some limitations.Because the FGLG mutations and overexpressing cFLIP tDED suppress Casp-8 tDED self-filamentation in reducing sample heterogeneity and trapping a homogeneous minimum complex, our structures would not be 100% identical to the corresponding, diverse native complexes obtained from cells.Our structure could only suggest possible DED-DED interactions within the complexes.Additionally, our structures couldn't reveal interactions between Casp-8 tDED trimers, the dimerization of Casp-8's protease domain, the complete structure of FADD because the protease domain as well as FADD DD remain invisible.However, these aspects have been addressed in prior studies 38,39,51,[75][76][77][78] .Furthermore, future investigations are necessary to investigate whether cFLIP could effectively impede full Casp-8 activation if cFLIP doesn't target FADD and the first CBS on the FADD-Casp-8 intermediate complex.
In addition to our investigations into multiprotein FADD-Casp-8-cFLIP DED complexes, it is noteworthy to mention recently reported domain-swapped dimer formations in Casp-8 tDED under specific conditions, involving the F122A mutation or a two-residue truncation possibly at the C-terminus of DED2's H6 51,77 .The details of Casp-8 tDED domain-swapping merit consideration in the broader context  11g.Each asymmetric unit is highlighted by thick lines.Two asymmetric units, for example, the N th and (N + 1) th , of the Casp-8 filament assemble a Casp-8 double layer and hence a CBS, stabilizing the first Casp-8 tDED (black) of the next forming (N + 2) th asymmetric unit.This arrangement allows its protease domain and the protease domain of the third Casp-8 tDED located in the N th asymmetric unit to form an apoptotic dimer (depicted as red balls).See also Supplementary Fig. 11f, g for apoptotic Casp-8 formation.
of DED assembly dynamics, a topic that may be explored in future studies.In a broader context of DD-fold multiprotein assembly, we found the diverse use of various CSS in self-assembly in other DDfold multiprotein structures.For example, the RIG-I tandem CARD assembly 79 utilizes a type III-I-III CSS (comprising one type I and two type III surfaces) to self-assemble a tetramer (Supplementary Fig. 14d).In the human apoptosome 79 , the heterodimeric Apaf-1-Casp-9 CARD protomer employs a type III-II-III CSS to self-assemble a trimer (Supplementary Fig. 14e).In our study, the interaction of two single FADD DED molecules leads to a homodimer that creates a type-III-II-III CSS surface to bind Casp-8 tDED , supporting our earlier hypothesis 80 .
The structural insights provided in this study, elucidating previously undocumented interactions such as FADD DED -FADD DED , FADD DED -Casp-8 tDED , FADD DED -cFLIP tDED , Casp-8 tDED -cFLIP tDED , and cFLIP tDED -cFLIP tDED within the ternary complex at a 3.7 Å resolution, mark a pivotal advancement in our comprehension of the intricate multiprotein DED/tDED assembly in 3D.By unveiling crucial determinants of specificity in assembling a complex with pseudo-helical symmetry, these structural data propel our insights to a higher dimension.The revelation underscores the imperative for further research to uncover the functional implications embedded in these intricate structural findings, especially in different types of cells with variations in receptor levels, signaling molecules, regulatory mechanisms, and unique genetic defects.

Protein crystallization
The protein complex was crystallized at a protein concentration of 10 mg/mL by the hanging-drop vapor-diffusion method at 20 °C with a solution of mixing 100 mM Na-HEPES at pH 7.0, 100 mM TBG at pH 9.0, 8% PEG8000, and 10 mM TCEP at pH 7.3.The SeMet-substituted protein complex was crystallized by the same hanging-drop vapordiffusion method.The SeMet-substituted protein crystals was crystallized by using a solution containing 92 mM Na-HEPES at pH 7.0, 169 mM TBG at pH 9.0, 8% PEG8000, and 9 mM TCEP at pH 7.3.

Crystal structure determination and model building
Anomalous and native diffraction data was collected at the beamline TLS BL13B1 at NSRRC, using the wavelengths of 0.97939 and 0.99984 Å, respectively, at 110 K.The data sets were processed using the program HKL-2000.The structure of the FA FuL_H9G -C8 FGLG -CF H7G complex was determined by using a SeMet-derivative dataset and the MR-SAD method in Phenix ver 1.14-3260.There was one 1:5:4 FA FuL_H9G -C8 tDED_FGLG -CF tDED_H7G complex per asymmetric unit with a solvent content of 65%.The structural model was iteratively built and refined using the programs Coot ver 0.8.9.1 EL and Phenix ver 1.14-3260, respectively.There is no electron density for FADD DD.All residues belong to the Ramachandran favored and allowed regions with no outliers in both structures.Data collection and refinement statistics were summarized in Supplementary Table 1.

The ball-and-ribbon diagram
In Figs.2b and d, the ball-and-ribbon diagrams show the spatial relationship of individual DEDs of the ternary complexes by using the PyMOL program ver 1.8.2.1 to draw ribbons that connect the spatially conserved Cα atoms (shown as balls) of every two adjacent DEDs.The ribbons show that DEDs assemble via the type I, II, and also III interfaces: blue, green, and cyan ribbons represent the DED assembly through the type I interface (called the type I connectivity), while gray ribbons represent the DED assembly through the type II interface (the type II connectivity).Red, yellow, and pink ribbons represent the DED assembly through the type III interface (the type III connectivity).The balls are the Cα atoms of the spatially conserved leucine residues among DEDs including FADD residue L63, Casp-8 residues L62 and L162, and cFLIP residues L55 and L152 (Supplementary Fig. 1c).In addition, the spatially conserved Cα atoms were also used to calculate the helical twist shown in Fig. 5c by the HELANAL-Plus program (https://dna.mbu.iisc.ac.in/resources.htm).

Multi-angle light scattering
In the SEC-MALS experiments, ternary DED complexes were injected onto a Superdex 200 (5/150) size-exclusion column and a Wyatt protein SEC column with the pore size of 300 Å, respectively.The SEC column was equilibrated with 20 mM Tris (pH 8.0) and 80 mM NaCl at room temperature, through a fast protein liquid chromatography system (Äkta purifier 10) coupled with a three-angle light-scattering detector (mini-DAWN TREOS) and a refractive index detector (Optilab T-rEX) (Wyatt Technology).Data analysis was carried out using the program ASTRA ver 6.0.5.3.

Small-angle X-ray scattering
In the SEC-SAXS experiments, the SAXS data was collected at the SWAXS beamline BL23A1 at NSRRC with an online size-exclusion highperformance liquid chromatographic system (Agilent chromatographic system 1260 series).Each protein sample was injected into an Agilent Bio SEC-5 HPLC column with a flow rate of 0.35 ml/min.Once the complex is eluted, the solution will go through a quartz capillary (2.0 mm diameter) with a flow rate decreased to 0.03 ml/min for the SAXS data collected with 30 s per frame using a Pilatus 1M-F area detector.All buffer solutions were measured under the same condition for background scattering subtraction.The SAXS data was analyzed by the ATSAS program suite ver 2.7 to 3.2.1.Data collection and structural parameters were summarized in Supplementary Table 2.

Treatment of protein precipitates for EM studies
The precipitates of overexpressed wild-type protein or complexes were resuspended in water for negative stain EM studies.

Negative staining
In all, 4 μl sample solution was applied onto the carbon-coated side of a TEM carbon type-B grid (Ted Pella, 01814-F) for 30 seconds and then the liquid was drawn off from the edge of grid with a filter paper (Whatman).Immediately, 4 μl of 1% uranyl acetate or uranyl formate was applied to the grid for 30 seconds and drawn off with a filter paper.Then the grid was placed into an electronic dry cabinet to air dry before imaging, which uses a FEI Tecnai G2 F20 S-TWIN at ICOB, Academia Sinica.To detect His-tagged targets, 5 nm Ni-NTA Nanogold was used according to Supplier's instruction (Nanoprobes).

Protein sample cross-linking
We utilized the gradient-based cross-linking method, also called the GraFix method, for protein sample cross-linking.Before cross-linking, purified protein complexes were dialyzed against a HEPES buffer and then concentrated to 1 mg/ml.For creating gradients of 10-30% glycerol with 0.016-0.05%glutaraldehyde, a centrifuge tube (14 × 89 mm, Beckman Coulter) containing a top solution (80 mM NaCl, 20 mM HEPES pH 8, 10% glycerol) and a bottom solution (80 mM NaCl, 20 mM HEPES pH 8, 30% glycerol, 0.05% glutaraldehyde) was placed into a gradient mixer (the Gradient Master 108, BioComp Instrument).Subsequently, a 200-μl buffering cushion (80 mM NaCl, 20 mM HEPES pH 8, 7% glycerol) was added on the top of the gradient, followed by loading a 200-μl protein sample on the top of the cushion.The ultracentrifugation was carried out at 4 °C in a swing-out rotor (SW-41, Beckmann) at a speed of 273,620 × g or 40,000 rpm for 18.5 h.The gradient was then fractionated from the bottom and each fraction was analyzed by SDS-PAGE (Bio-Rad).The peak fractions were further loaded onto a prewashed desalting column (Zeba TM Spin Desalting Columns, Thermo Scientific) to remove glycerol and excess cross linkers.The cross-linked complex was eluted in a TRIS buffer (80 mM NaCl, 20 mM Tris pH 8) and stored at 4 °C.

Cryo-EM grids preparation and data acquisition
The glutaraldehyde cross-linked protein samples (~250 μg/ml) (Complex B) were applied to glow-discharged holey carbon grids (Quantifoil Cu, R1.2/1.3, 300 mesh).Each grid was blotted for 3 ~4 s and flashplunged into liquid ethane pre-cooled in liquid nitrogen using an FEI Vitrobot mark IV operated at 4 °C and 100% humidity.Cryo-EM data were acquired on a Titan Krios (FEI) operated at 300 kV, equipped with a Gatan K2 Summit detector at ASCEM, Academia Sinica.The EPU software was utilized for automated data collection.Movies were collected at a nominal magnification of 165,000× in counting mode resulting in a calibrated pixel size of 0.84 Å/pixel, with a defocus range of approximately -0.5 to -2.5 μm.Eighty frames were recorded over 6 s of exposure at a dose rate of 0.9 electrons per Å 2 per frame.Data collection, refinement and validation statistics were summarized in Supplementary Table 3.
The non-crosslinked protein sample (Complex A) was absorbed onto freshly glow-discharged Quantifoil 2/1 grids with PELCO easiGlow glow discharger and flash frozen in liquid ethane using Leica GP Climate controlled sample plunger with a controlled temperature and humidity.Cryo-EM movies were collected with FEI Talos Arctica electron microscope equipped with a Gatan BioQuatum energy filter and a K2 Summit direct electron detector at the Institute for Quantitative Biomedicine at Rutgers University, USA using the software EPU for automated data collection.We collected 30 movie frames with a combined exposure time of 7.5 s corresponding to a total dose of 24 electrons per Å 2 (0.8 electrons/frame).Defocus values were set from −0.5 to −3 μm at a magnification of 130,000 times resulting with a pixel size of 1 Å.

Cryo-EM image processing and model refinement
All datasets were processed using the CryoSparc V2 software package installed in our own computers.Movie frames were aligned by running the job Full-frame motion correction.The contrast transfer function parameters for each aligned micrograph were estimated by running CTF estimation (CTFFIND4).Particle templates were created from the particles picked manually from 15 to 20 micrographs.Particles were then picked automatically by running Template picker.All particles were local-aligned and extracted by running Local motion correction, and then subjected to 2D classification for several cycles to remove junk particles.Ab initio 3D classification was carried out by running Ab-initio Reconstruction.After removing junk particles, the jobs the heterogeneous refinement, homogeneous refinement, and non-uniform refinement were performed.All maps were sharpened and the resolution was estimated using the Fourier shell correlation (FSC) = 0.143 cutoff criterion (Supplementary Figs. 5 and 6).
The crystal structures of FADD DED , cFLIP tDED , and C8 tDED , were fit into the Cryo-EM envelops using UCSF Chimera ver 1.13.1 and refined in real space using the Phenix ver 1.14-3260 software.Identification of Casp-8 and cFLIP is facilitated by the presence of envelops for helix H7 of tDED, with further confirmation of cFLIP identity through the observation of disordered helix H3 in both cFLIP DED1 and DED2 (Supplementary Figs.1c and 9).Notably, given that tDED but not FADD DED has helix H7 (Supplementary Fig. 1a and Supplementary Figs. 8, 9, vs 7), the absence of an envelope for helix H7 of tDED distinctly indicates that in Complex B, the position typically occupied by the tDED of C8d is instead taken up by two FADD DED molecules (Supplementary Fig. 2e).The Casp-8 protease domain and FADD DD were not visible.

Mutagenesis and pulldown assays
All gene mutations were generated by using the KOD Plus Mutagenesis Kit (TOYOBO) or In-Fusion HD Cloning Plus kit (TaKaRa).The Histagged proteins were expressed and captured by the resin (Qiagen).Excess proteins and impurities were removed by three times of wash with 40 mM imidazole.The resin was then mixed with non-tagged protein lysates at room temperature for 1 h, and then washed again with three times of 40 mM imidazole.The proteins were eluted with 1 M imidazole.All samples are subjected to SDS-PAGE analysis with Coomassie blue staining.The mutagenesis primers are listed in Supplementary Table 4.

Generation of FADD knockout cells
SgRNA targeting on FADD and pAll-Cas9.pPuroplasmid were designed and purchased from the National RNAi Core Facility at Academia Sinica, Taiwan.iMEF was transfected with CRISPR plasmid using Turbofect (Thermo) according to manufacturer's instructions.On the third day after transfection, iMEF underwent serial dilutions and antibiotic selection to remove unwanted cells.Surviving cell colonies were examined by western blotting to confirm the gene knockout (Supplementary Fig. 15a).The FADD-gene knockout colonies were expanded and stored for the following experiments.FADD-KO clone sg4.B9 was used for expansion because necroptotic signaling molecules MLKL and RIPK3 remain there (Supplementary Fig. 15a).TNF-induced NF-κB activation signaling remains normal in the FADD-KO iMEF cells (clone sg4.B9) with or without CHX (Supplementary Fig. 15g, h).The FADDgene knockout HAP1 (RRID:CVCL_SM74) in Fig. 6g were purchased from Horizon Discovery.

FADD reconstitution
The human or mouse full-length FADD gene was cloned into the pAS4.1w.Pbsd-aOn vector.HEK293T cells (American Type Culture Collection (ATCC) CRL-3216, RRID:CVCL_0063) were transfected with FADD constructs and the packaging plasmids pMD.G and pCMVR8.91(the National RNAi Core Facility at Academia Sinica) with Turbofect according to manufacturer's instructions.Virus-containing mediums were harvested 48 and 72 h after transfection.FADD-gene knockout iMEF clone was incubated with the virus-containing medium overnight for infection.After infection, iMEF were selected with blasticidin (5 μg/ ml) to eliminate uninfected cells.For HAP1 cells, 7.5 μg/ml blasticidin was used.Stable colonies were then saved for following assays.FADD protein expression was induced by doxycycline hyclate (0.1-1 μg/ml) for 16-24 h before additional treatments.The cloning primers are listed in Supplementary Table 4.

Cell-based mutagenesis assays
Tet-inducible plasmids containing FADD WT or mutant sequences were transfected into FADD-deficient immortalized mouse embryonic fibroblast (FADD -/-iMEF) using a lentivirus packaging system.Mouse FADD (mFADD)-reconstituted iMEF were treated with doxycycline overnight to induce FADD expression.iMEF were seeded and grew to reach 60-80% confluence before assays.To induce apoptosis, iMEF were pretreated with cycloheximide (CHX, 10 μg/ml) for 30 min, followed by the stimulation with recombinant mouse TNFα (10 ng/ml) for 6 h or the indicated time.For necroptosis induction, iMEF were pretreated with cycloheximide (10 μg/ml) and z-VAD-fmk (50 μM), before TNFα treatment.Human FADD (hFADD)reconstituted HAP1 cells were treated with doxycycline overnight to induce FADD expression.To induce apoptosis in HAP1 cell, HAP1 cells were pretreated with cycloheximide (10 μg/ml) for 30 min, followed by the stimulation with SuperKillerTRAIL (50 ng/ml).All the mutants were created by KOD-based site-direct mutagenesis by using the primers listed in Supplementary Table 4. Uncropped data are included in a Source Data file.

Fluorescence apoptosis and Necrosis assay
iMEFs were seeded in a 96-well plate (5000 cell per well) a day before the assay.To induce apoptosis, iMEF were pretreated with cycloheximide (CHX, 10 μg/ml) for 30 min, followed by the stimulation with recombinant mouse TNFα (10 ng/ml) for 6 h or the indicated time.For necroptosis induction, iMEF were pretreated with cycloheximide (10 μg/ml) and z-VAD-fmk (50 μM), before TNFα treatment.Nucleic acid and the Casp-3 activity were detected by using SYTO green (5 μM) and DEVD-AMC (20 μM), respectively.Fluorescent signal was detected by a 96-well plate reader (Victor X, PerkinElmer) at the time indicated in the figures and the data was analyzed.Bar chars were generated by GraphPad Prism 9.4.1.Notably, this assay was modified from a previous assay 82 .

Cell lysate-based mutagenesis study
In vitro mutagenesis experiments to test FADD-mediated signaling were performed by a HeLa cell lysate-based protein expression system (1-Step Human Coupled IVT kit, Thermo).The full-length wild type and mutant FADD proteins were expressed by PURExpress in vitro protein synthesis kit (NEB) using pET-26 vector.The reaction mixture with expressed FADD protein was added to the reaction component of the IVT kit to a final FADD concentration of about 4 μM (measured by UV absorbance), higher than ~0.33 μM of endogenous FADD 83 .The mixture was incubated at 30 °C for 6 h and then was analyzed by SDS-PAGE and western blotting.All the mutants were created by KOD-based sitedirect mutagenesis by using the primers listed in Supplementary Table 4. Uncropped data are included in a Source Data file.

Reporting summary
Further information on research design is available in the Nature Portfolio Reporting Summary linked to this article.

Fig. 1 |
Fig. 1 | Casp-8 tDED mutations impair Casp-8 self-filamentation but facilitate complex reconstitution.a The wild-type (WT) Casp-8 tDED (C8) predominantly forms filaments.Negative-stain electron microscopy (EM) and Coomassie bluestained SDS-PAGE analysis of precipitates formed by the wild-type protein or complexes and resuspended in water.White arrowheads indicate some His-tagged proteins detected by Nanogold.Sample 1: WT Casp-8 tDED with a C-terminal His-tag (WT C8 C-tag).Sample 2: WT Casp-8 tDED plus WT cFLIP tDED with an N-terminal His-tag (WT CF N-tag).Sample 3: WT Casp-8 tDED plus WT FADD with a C-tag.b Casp-8 tDED_F122A mutant aids in the reconstitution of soluble DED complexes.SEC profile of the binary CF H7G -Casp-8 tDED_F122A complex and negative-stain EM and SDS-PAGE analyses of the peak fractions.AU absorbance units.c Monomeric Casp-8 tDED_F122G/L123G mutant (C8 FGLG ) forms short filaments in the presence of WT FADD.Negative-stain EM images show that C8 FGLG purified by SEC cannot form filaments, whereas it forms short filaments in the presence of WT FADD, although FADD mostly dissociated.White arrowheads indicate C-terminal His-tagged (C-tag) FADD detected by Nanogold.The SDS-PAGE analysis of the EM sample of the binary complex is also shown.All micrograph and biochemical data were repeated independently twice with similar results.Scale bar = 50 nm.Source data are provided as a Source Data file.

Fig. 2 |
Fig. 2 | FADD, Casp-8, and cFLIP assemble a single-and a triple-FADD complexes.a-c The ribbon, ball-and-ribbon, and hexagon diagrams in a-c, respectively, depict the crystal structure of the single-FADD ternary complex.In a and c, the FADD and Casp-8 portions are highlighted by red and white thick lines, respectively.In b, the diagram shows the type I, II, and III connectivity by ribbons connecting every two adjacent DEDs, represented by balls (Supplementary Fig. 1c, "Methods" section).In b and c, a red dashed circle indicates the adjoining space of Casp-8 molecule C8e, while a long black arrow with a red X indicates the space was not filled by any DED.Each hexagon in the 2D representation represents a DED, with six sides representing the type I, II, and III surfaces.Each protein or tDED molecule is labeled with its chain ID and colored uniquely.CFk1, for example, stands for the DED1 of cFLIP (CF) with the chain ID k.The molecule with the same chain ID retains consistent coloring across all three diagrams to facilitate comparison and identification, except that Casp-8 and cFLIP are colored in green and blue, respectively, in d and Fig. 7b.The dashed hexagons, which adjoin the tDED with the solid lines, represent an adjacent tDED from a different layer.The angled and angled/dashed lines highlight the CSS of tDEDs with solid edges and dashed edges, respectively.Notably, cFLIP and Casp-8 CSS are colored in green and pink, respectively.Top and bottom ends, see Supplementary Fig. 13.d-f Similar to a-c, except that the diagrams d-f depict the cryo-EM structure of the triple-FADD ternary complex.Long black arrows with a red X indicate that FADD physically blocks Casp-8 filamentation on the top end.g Shows a type III interaction between cFLIP tDED and Casp-8 tDED , colored in pink and green, respectively.

Fig. 3 |
Fig. 3 | Casp-8 tDED utilizes the type III-II-III CSS to self-assemble in both intermediate complexes.a Shows the single-FADD-Casp-8 intermediate complex derived from the single-FADD ternary complex structure by removing cFLIP.FADD DED , as ribbons, and Casp-8 tDED , as molecular surfaces, are labeled and colored as in Fig. 2a.Type Ia, IIb, IIIa, and IIIb surfaces of Casp-8 tDED are colored in yellow, green, red, and blue, respectively, similar to those in Supplementary Fig. 1.However, for clarity, the type Ib surface of Casp-8 tDED molecule C8a is colored in gray, while type IIa surfaces of Casp-8 DED1 and DED2 are colored in orange and black, respectively.b Similar to a, except that here shows the triple-FADD-Casp-8 intermediate complex derived from the triple-FADD ternary complex structure.c Sideby-side comparison of the assembly of the single-and triple-FADD-Casp-8 intermediate complexes.The comparison reveals that Casp-8 tDED assembles consistently via CSS, which is highlighted in magenta.Additionally, the lower parts of two intermediate complexes consistently contain FADD DED molecule FAl and Casp-8 tDED molecules C8a-c.However, in the upper part of the triple-FADD complex, FADD DED molecules FAq and FAr could together assemble a surface mimicking the CSSa of the Casp-8 tDED molecule C8d in the single-FADD complex, also explained in d. d Structural comparison between the single-FADD-single-Casp-8 assembly, i.e., the FAl-C8d assembly, in a and the triple-FADD assembly in b by superimposing FADD DED molecule FAl.The comparison reveals that FADD DED molecules FAq and FAr could assemble like a Casp-8 tDED molecule C8d and hence form a surface that mimics CSSa in c.

Fig. 4 |
Fig. 4 | FADD DED -FADD DED and FADD DED -Casp-8 tDED assemblies in the intermediate complex.a Shows that FADD DED molecules FAl, FAr, and FAq assemble a right-handed trimer that binds a left-handed Casp-8 tDED trimer in the triple-FADD-Casp-8 intermediate complex.The molecules are labeled and colored as in Fig. 3a, b.FAq and FAr refer to FADD DED (FA) with the chain ID q and r, respectively.b Shows the interface residues on type I FADD DED -FADD DED and FADD DED -Casp-8 tDED interfaces.The green and pink boxes show the residues on the type I interfaces in the triple-FADD, i.e., the FAl-FAr-FAq assembly, while the purple box shows the interface residues between Casp-8 tDED molecule C8a and FADD DED molecule FAl.The type Ia surfaces and corresponding ribbons of FADD DED are colored in yellow.The interface residues of FADD DED molecules FAl, FAr, and FAq are labeled in red, purple, and black, respectively.while those on Casp-8 tDED molecule C8a are labeled in black.c, d Black boxes and double-headed arrows highlight the CSSb-CSSa interaction between the Casp-8 tDED trimer (c) and FADD DED trimer (d) of the triple-FADD complex.In d, type IIa and IIIa surfaces are colored in black and red, respectively, in which functionally important FADD residues K33 and E51 are highlighted in white.The size of each interface on FADD DED is shown in parentheses.Notably, in c, the type Ib residues of Casp-8 tDED molecule C8a are labeled in black.e-f, Black boxes and double-headed arrows highlight the corresponding CSSb-CSSa interaction in the single-FADD complex, between the corresponding Casp-8 tDED trimer (e) and single-FADD-single-Casp-8 assembly (f) with similar orientations to the those in c and d, respectively.Notably, in f, Casp-8 surfaces are colored as in Fig. 3a, except that functionally important Casp-8 residues R33 and K148 38 have white surfaces.

Fig. 5 |
Fig. 5 | cFLIP targets the CBS of the FADD-Casp-8 intermediate complex and further caps it.a Thick orange lines highlight the CBS of the single-FADD intermediate complex shown in 2D representation.The CBS is targeted by cFLIP tDED molecule CFk, as the first step of cFLIP recruitment.b Thick orange lines highlight the CBS generated after the recruitment of cFLIP tDED molecule CFk to the single-FADD complex.The CBS could recruit another cFLIP tDED molecule CFj.This process repeats until the complex is capped by cFLIP and reaches a maximum capacity of four cFLIP molecules.c Shows FADD DED -cFLIP tDED and Casp-8 tDED -cFLIP tDED assemblies in the single-FADD complex.Surface representations of the single-FADD intermediate complex viewed from different angles show that the CBS contains a type Ia surface (yellow) from Casp-8 tDED molecule C8c DED1, a type IIa surface (orange) from Casp-8 tDED molecule C8d DED1, a type IIa (black) and a type IIIa (red) surfaces from FADD DED molecule FAl, and a type IIIa surface (red) from Casp-8 tDED molecule C8a DED2.Red balls in the middle panel indicate the possible locations of the protease domains.d The pink box highlights FADD DED -cFLIP tDED and Casp-8 tDED -cFLIP tDED interactions in c. cFLIP tDED molecule CFk is shown as pink ribbons, while its interface residues are shown as sticks.In c-e, FADD DED and Casp-8 tDED are labeled and colored as in Fig. 2a, except that FADD DED molecule FAl is colored in white for clarity and for the comparison with the white Casp-8 tDED molecule in f. e The pink box highlights the corresponding CBS surfaces in the triple-FADD intermediate complex.Notably, two type IIa surfaces (black) are from FADD DED molecules FAl and FAr.f, The corresponding CBS surfaces in the C8 filament (5L08 [https://doi.org/10.2210/pdb5L08/pdb]) 38 .White surfaces highlight the C8 molecule that provides two type IIa (black and orange) and a type IIIa (red) surfaces.

Fig. 6 |
Fig. 6 | Roles of the triple-and single-FADD models in hierarchical apoptotic signaling.a Show five interfaces between FADD DED and tDED in the single-FADD structure.The interface residues of FADD are label in red, while FADD residues for mutagenesis are in red boxes.The side chains of the interface residues of FADD are shown as ball-and-sticks, while those of Casp-8 and cFLIP are shown as sticks.The interface residues of Casp-8 are colored as in Fig. 3a, while those of cFLIP are colored as in Supplementary Fig. 1a, respectively.The helices are numbered in Supplementary Fig. 2e.b Cell-based mutagenesis assays.FADD-reconstituted iMEF cells were treated with TNF/CHX (TC) to trigger apoptotic signaling.T TNFα, C CHX, Vec empty vecto, doxy doxycycline.F25R, K33E, and E51R mutants are highlighted in red because they are inactive in Supplementary Fig. 15c-f.c Same as b, but treated with TNF/CHX/ zVAD (TCZ) to inhibit caspase activity and promote necroptotic signaling.Z zVAD.d Same as b, but FADD-reconstituted HAP1 cells were treated with TRAIL/CHX.All cell-based experiments were repeated twice with similar results.Uncropped blots are provided as a Source Data file.

Fig. 7 |
Fig. 7 | DED assembly mechanisms in regulating apoptotic signaling.a, b Propose a hierarchical FADD-mediated DED assembly mechanism for the FADD-Casp-8 and FADD-Casp-8-cFLIP complexes.a In the first stage, the formation of a FADD-Casp-8 intermediate complex requires CSS-mediated self-assembly of endogenous Casp-8 and also a high local concentration of FADD to interact with the Casp-8 assembly.Notably, the single-FADD intermediate complex assembles in a similar manner.b In the second stage, cFLIP targets the CBS on the intermediate complex, terminating hierarchical apoptotic signaling.This process generates a Casp-8-cFLIP hetero-double layer, licensing local Casp-8 activation.However, when cFLIP is depleted, Casp-8 binds the same CBS, forming Casp-8 double layers and hence filaments to execute apoptosis.This unveils structurally how the levels of cFLIP mechanically regulate apoptotic signaling.c A 2D representation illustrates tDED assembly in a Casp-8 filament, elucidating the mechanism of generating apoptotic Casp-8.The tDED is colored as per the suggested model for EMD-11939 in Supplementary Fig.11g.Each asymmetric unit is highlighted by thick lines.Two asymmetric units, for example, the N th and (N + 1) th , of the Casp-8 filament assemble a Casp-8 double layer and hence a CBS, stabilizing the first Casp-8 tDED (black) of the next forming (N + 2) th asymmetric unit.This arrangement allows its protease domain and the protease domain of the third Casp-8 tDED located in the N th asymmetric unit to form an apoptotic dimer (depicted as red balls).See also Supplementary Fig.11f, g for apoptotic Casp-8 formation.